This web page is for demonstration/small dataset only. Please use small dataset as it may take long time to execute. For large read files please download stand-alone from downloadtab
To convert your fastq file to tab separated file having unique reads and count, please download this program Extract.zip.

Upload file with unique reads and their count in tab separated format:

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server load 1%

OR

Paste reads with their count in tab separated format :

Try this example:

Select the model species:

Number of processors:

Please read the detailed information before using the program on help page

(Optional : Use filter options to reduce computation time. Chosen filter will reduce number of sequences to process. To know more about filters option please read the details given below. Use of filters might compromise accuracy of the classifier)